Protein Extraction and Immunoblotting

Proteins were extracted from adherent cells and separated as previously described^{18 (link)}. Primary antibodies were as following: MGMT clone MT3.1 (#NB 100–692 Novus, MO) and anti-actin (clone C4, MAB1501 Millipore). Peroxydase-conjugated secondary antibodies (Jackson Immunoresearch Laboratories, PA) were detected using the ECL detection system (Amersham Biosciences, NJ) (N = 3).

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Rabé M., Dumont S., Álvarez-Arenas A., Janati H., Belmonte-Beitia J., Calvo G.F., Thibault-Carpentier C., Séry Q., Chauvin C., Joalland N., Briand F., Blandin S., Scotet E., Pecqueur C., Clairambault J., Oliver L., Perez-Garcia V., Nadaradjane A., Cartron P.F., Gratas C, & Vallette F.M. (2020). Identification of a transient state during the acquisition of temozolomide resistance in glioblastoma. Cell Death & Disease, 11(1), 19.

Publication 2020

anti-actin (clone C4 Peroxydase-conjugated secondary antibodies ECL detection system

Actin Antibodies Clone Mgmt Novus Proteins

Corresponding Organization :

Other organizations : Inserm, Université d'Angers, Nantes Université, University of Castilla-La Mancha, Sorbonne Université, Laboratoire Jacques-Louis Lions, Université de Strasbourg, Institut de génétique et de biologie moléculaire et cellulaire, Centre National de la Recherche Scientifique, Institut de Cancérologie de l'Ouest

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Variable analysis

independent variables

None explicitly mentioned

dependent variables

Protein expression levels of MGMT and actin

control variables

Number of adherent cells from which proteins were extracted
Protein extraction and separation method as previously described in ref. 18
Primary antibodies used: MGMT clone MT3.1 and anti-actin (clone C4)
Peroxydase-conjugated secondary antibodies detected using the ECL detection system

controls

Positive control: Not specified
Negative control: Not specified

Annotations

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